Please use this identifier to cite or link to this item: http://hdl.handle.net/10397/103862
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dc.contributorDepartment of Biomedical Engineering-
dc.creatorCui, Xen_US
dc.creatorLiu, Len_US
dc.creatorLi, JYen_US
dc.creatorLiu, Yen_US
dc.creatorLiu, Yen_US
dc.creatorHu, Den_US
dc.creatorZhang, Ren_US
dc.creatorHuang, Sen_US
dc.creatorJiang, Zen_US
dc.creatorWang, Yen_US
dc.creatorQu, Yen_US
dc.creatorPang, SWen_US
dc.creatorLam, RHWen_US
dc.date.accessioned2024-01-10T02:41:03Z-
dc.date.available2024-01-10T02:41:03Z-
dc.identifier.urihttp://hdl.handle.net/10397/103862-
dc.language.isoenen_US
dc.publisherMDPI AGen_US
dc.rights© 2022 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).en_US
dc.rightsThe following publication Cui, X., Liu, L., Li, J., Liu, Y., Liu, Y., Hu, D., ... & Lam, R. H. (2022). A Microfluidic Platform Revealing Interactions between Leukocytes and Cancer Cells on Topographic Micropatterns. Biosensors, 12(11), 963 is available at https://doi.org/10.3390/bios12110963.en_US
dc.subjectLive-cell immunoassayen_US
dc.subjectTopographic micropatternsen_US
dc.subjectOn-chip cytokine detectionen_US
dc.subjectNasopharyngeal canceren_US
dc.subjectIntegrated microfluidicsen_US
dc.titleA microfluidic platform revealing interactions between leukocytes and cancer cells on topographic micropatternsen_US
dc.typeJournal/Magazine Articleen_US
dc.identifier.volume12en_US
dc.identifier.issue11en_US
dc.identifier.doi10.3390/bios12110963en_US
dcterms.abstractImmunoassay for detailed analysis of immune-cancer intercellular interactions can achieve more promising diagnosis and treatment strategies for cancers including nasopharyngeal cancer (NPC). In this study, we report a microfluidic live-cell immunoassay integrated with a microtopographic environment to meet the rising demand for monitoring intercellular interactions in different tumor microenvironments. The developed assay allows: (1) coculture of immune cells and cancer cells on tunable (flat or micrograting) substrates, (2) simultaneous detection of different cytokines in a wide working range of 5-5000 pg/mL, and (3) investigation of migration behaviors of mono- and co-cultured cells on flat/grating platforms for revealing the topography-induced intercellular and cytokine responses. Cytokine monitoring was achieved on-chip by implementing a sensitive and selective microbead-based sandwich assay with an antibody on microbeads, target cytokines, and the matching fluorescent-conjugated detection antibody in an array of active peristaltic mixer-assisted cytokine detection microchambers. Moreover, this immunoassay requires a low sample volume down to 0.5 mu L and short assay time (30 min) for on-chip cytokine quantifications. We validated the biocompatibility of the co-culture strategy between immune cells and NPC cells and compared the different immunological states of undifferentiated THP-1 monocytic cells or PMA-differentiated THP-1 macrophages co-culturing with NP460 and NPC43 on topographical and planar substrates, respectively. Hence, the integrated microfluidic platform provides an efficient, broad-range and precise on-chip cytokine detection approach, eliminates the manual sampling procedures and allows on-chip continuous cytokine monitoring without perturbing intercellular microenvironments on different topographical ECM substrates, which has the potential of providing clinical significance in early immune diagnosis, personalized immunotherapy, and precision medicine.-
dcterms.accessRightsopen accessen_US
dcterms.bibliographicCitationBiosensors, Nov. 2022, v. 12, no. 11, 963en_US
dcterms.isPartOfBiosensorsen_US
dcterms.issued2022-11-
dc.identifier.isiWOS:000894830300001-
dc.identifier.scopus2-s2.0-85141891501-
dc.identifier.pmid36354472-
dc.identifier.eissn2079-6374en_US
dc.identifier.artn963en_US
dc.description.validate202401 bcvc-
dc.description.oaVersion of Recorden_US
dc.description.fundingSourceRGCen_US
dc.description.fundingSourceOthersen_US
dc.description.fundingTextGeneral Research Grant of Hong Kong; Natural Science Foundation of Guangdong Provinceen_US
dc.description.pubStatusPublisheden_US
dc.description.oaCategoryCCen_US
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